Activity of four cry gene promoters in spoIIID mutant of Bacillus thuringiensis
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Supported by Key Project of Chinese National Programs for Fundamental Research and Development (2009CB118902) and by the National Natural Science Foundation of China (31070083)

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    Abstract:

    Abstract:[Objective]We studied the influence of spoIIID gene deletion on the activity of cry1Ac,cry3A,cry4A and cry8E gene promoters in Bacillus thuringiensis and compared the activity among these promoters in spoIIID mutant (HD-!SpoIIID). [Methods]We constructed 4 promoter fusions with lacZ gene and transformed them into wild-type strain HD-73 and HD-!SpoIIID to analyze their transcriptional activity. We constructed a spoIIID gene mutant (HD - -!SpoIIID)with deletion of the cry1Ac-harboring native plasmid based on HD-!SpoIIID strain. We constructed four promoter fusions with cry1Ac gene and transformed them into HD-ΔSpoIIID and HD - -ΔSpoIIID to perform Cry protein quantization and bioassay. [Results]By Beta-galactosidase assay we found that the activities of the four promoters were,in decreasing order,Pcry8E > Pcry1A > Pcry4A > Pcry3A in both HD-73 and HD-ΔSpoIIID strains. The deletion of spoIIID had no effect on transcriptional activity of Pcry1Ac and Pcry8E. The transcriptional activity of Pcry3A in HD-ΔSpoIIID was slightly higher than that in HD-73. The transcriptional activity of Pcry4A in HD-ΔSpoIIID was decreased compared to HD-73. The Cry1Ac protein production directed by Pcry1Ac was as much as Pcry8E in HD-ΔSpoIIID and higher than that by Pcry4A and Pcry3A in accordance with the bioassay result. [Conclusion]The cry8E gene promoter is the strongest promoter among four promoters in spoIIID gene mutant at transcriptional level. The Cry1Ac protein production directed by Pcry1Ac is almost equal to that by Pcry8E.

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Xinmei Wang, Lixin Du, Qi Peng, Yingping Liang, Jie Li, Jie Zhang, Fuping Song. Activity of four cry gene promoters in spoIIID mutant of Bacillus thuringiensis. [J]. Acta Microbiologica Sinica, 2012, 52(9): 1075-1084

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History
  • Received:April 05,2012
  • Revised:May 02,2012
  • Adopted:
  • Online: September 12,2012
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